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RAD52的显性负等位基因揭示了一个包含Rad51和Rad52的DNA修复/重组复合体。

Dominant negative alleles of RAD52 reveal a DNA repair/recombination complex including Rad51 and Rad52.

作者信息

Milne G T, Weaver D T

机构信息

Division of Tumor Immunology, Dana-Farber Cancer Institute, Boston, Massachusetts.

出版信息

Genes Dev. 1993 Sep;7(9):1755-65. doi: 10.1101/gad.7.9.1755.

Abstract

Saccharomyces cerevisiae rad52 mutants are characterized by severe defects in double-strand break (DSB) repair and recombination. In this study we have identified several regions of RAD52 that are required for these biological functions. We cloned and characterized a RAD52 homolog from Kluyveromyces lactis that partially complemented S. cerevisiae rad52 mutants while exhibiting negative dominance in wild-type (RAD52) strains. The dominant negative effect was suppressed by overexpression of RAD51, an additional gene known to be required for DSB repair and recombination, indicating a genetic interaction between these loci. Furthermore, GAL4 two-hybrid analysis revealed a physical interaction between Rad51 and the carboxy-terminal one-third of Rad52. Deletion alleles of rad52 (with or without the Rad51 association domain) also produced dominant negative defects, suggesting the disruption of repair through nonfunctional interactions with other DSB repair and recombination proteins. RAD51 relieved the negative dominance of each of these alleles either by competitive titration or functional activation of mutant or heterologous Rad52 proteins. These results demonstrate the importance of Rad52-Rad51 interactions and point to the formation of a higher order repair/recombination complex potentially containing other yet unidentified components.

摘要

酿酒酵母rad52突变体的特征是在双链断裂(DSB)修复和重组方面存在严重缺陷。在本研究中,我们鉴定了RAD52的几个对这些生物学功能至关重要的区域。我们从乳酸克鲁维酵母中克隆并鉴定了一个RAD52同源物,它部分互补酿酒酵母rad52突变体,同时在野生型(RAD52)菌株中表现出负显性。RAD51(另一个已知对DSB修复和重组必需的基因)的过表达抑制了这种显性负效应,表明这些基因座之间存在遗传相互作用。此外,GAL4双杂交分析揭示了Rad51与Rad52羧基末端三分之一之间存在物理相互作用。rad52的缺失等位基因(有或没有Rad51结合结构域)也产生显性负缺陷,这表明通过与其他DSB修复和重组蛋白的无功能相互作用破坏了修复。RAD51通过竞争性滴定或突变或异源Rad52蛋白的功能激活缓解了这些等位基因中的每一个的负显性。这些结果证明了Rad52-Rad51相互作用的重要性,并指出可能形成包含其他尚未鉴定成分的高阶修复/重组复合物。

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